Functional Interaction between Coactivators CBP/p300, PCAF, and Transcription Factor FKLF2

doi:10.1074/jbc.M108826200

Transcription and Nuclear Factor Monoclonals

Functional Interaction between Coactivators CBP/p300, PCAF, and Transcription Factor FKLF2^*

Chao-Zhong Song, Kimberly Keller, Ken Murata, Haruhiko Asano^§, and George Stamatoyannopoulos^¶

From the Division of Medical Genetics, Department of Medicine, University of Washington, Seattle, Washington 98195 and the ^§ First Department of Internal Medicine, Nagoya University, Nagoya 461-8673, Japan

Received for publication, September 13, 2001, and in revised form, December 7, 2001

ABSTRACT

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The Sp1/KLF family of factors regulates diverse cellular processes, including growth and development. Fetal Krüppel-likefactor (FKLF2) is a new member of this family. In this study,we characterized the coactivators involved in FKLF2 transcriptionalactivation. Our results show that both CBP/p300 and p300/CBP-associatedfactor (PCAF) enhance FKLF2 transcriptional activity. We demonstratethat the acetyltransferase activity of PCAF but not that of CBP/p300is required for stimulating FKLF2 transcription activity. We furthershow that p300 and PCAF act cooperatively in stimulating FKLF2transcriptional activation. FKLF2 interacts with both CBP andPCAF through specific domains, and CBP and PCAF acetylate FKLF2.Both CBP/p300 and PCAF stimulate FKLF2 DNA binding activity. Theintegrity of the acetyltransferase domain of PCAF but not thatof CBP/p300 is required for stimulating FKLF2 DNA binding activity.These results demonstrate that CBP/p300 and PCAF stimulate FKLF2transcriptional activity at least by enhancing its DNA binding.The acetyltransferase activities of CBP/p300 and PCAF play a distinctrole in stimulating FKLF2 transcription and DNAbinding.

INTRODUCTION

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The Sp1/KLF family of transcription factors regulates diverse cellular processes, including cell growth and differentiation,and is essential for early embryonic development (1-3). Thisfamily of proteins is characterized by the presence of three highlyhomologous C2H2 type zinc fingers near the C terminus that bindGC/GT boxes. Amino acid sequences in the transcription activation/repressiondomains are less conserved among family members. This family ofproteins exhibits a different affinity for the GC/GT boxes indifferent promoters and possesses transcriptional activation,repression, or both functions. Because the GC/GT boxes are oneof the most common regulatory elements in promoters of many cellularand viral genes, the characterization of the modulation of theirtranscriptional activities by different coactivators will providesignificant insight into the mechanism by which this family offactors regulates geneexpression.

Sp1 and EKLF,¹ an erythroid-specific factor that is required for the expression of the adult type $beta$ globin gene (4-7), arethe best studied in this family. EKLF interacts with CBP (8)as well as ERC-1 (EKLF coactivator remodeling complex 1). ERC-1is a SWI/SNF-related chromatin remodeling complex and is requiredfor generating a DNase I-hypersensitive, transcriptionally active $beta$ promoter on a chromatin template in vitro (9). EKLF was alsodemonstrated to interact with the corepressors mSin3A and HDAC1and repress transcription (10). The glutamine-rich activationdomain of Sp1 makes direct contact with the TAF110 subunit ofthe TFIID complex and mediates transcriptional activation (11).In addition, the transcriptional cofactor complex CRSP (cofactorrequired for Sp1 activation) has also been shown to be requiredfor Sp1 transcriptional activation in vitro (12).

CBP/p300 and PCAF function as coactivators for a variety of transcriptional activators and are involved in cell growth anddevelopment (13-17). CBP/p300 and PCAF have intrinsic histone acetylaseactivities (18-20). In addition to histone, a number of transcriptionfactors are also substrates for acetylation (15). The modificationof transcription factors by acetylation has been shown to regulatethe activation function at multiple levels, including DNA binding,interaction with other proteins, and stability (15). Despitethe general involvement of CBP/p300 and PCAF in transcriptionalactivation by many factors, recent studies suggest that differenttranscription factors show selective interaction with these coactivators,and the exact role of the acetylation of transcription factorsby these coactivators remains to beestablished.

FKLF2/RFLAT-1/BTEB3 (hereafter referred to as FKLF2) is a recently cloned member of the Sp1/KLF family of transcription factors(21-23). FKLF2 is a phosphorylated protein and is expressed ina variety of tissues (21-23). Our previous studies (21) haveshown that FKLF2 activates the human $gamma$ globin promoter and toa lesser degree the $epsilon$ and $beta$ globin promoters as well as severalerythroid-specific promoters. It also activates the SV40, SM22 $alpha$ ,and the RANTES (regulated on activation normal T cell expressedand secreted) gene promoter in transient assays (22, 23).DNA binding studies demonstrate that FKLF2 was able to bind toa consensus basic transcription element named BTE (22) and theA/B region of the RANTES gene promoter (23). Luciferase assaysusing reporter constructs containing different versions of the $gamma$ globin promoter have shown that, in addition to the CACCC sequenceat position $-$ 142, other regions including sequences surroundingthe TATA box in the $gamma$ globin promoter are also capable of mediatingFKLF2 transcriptional activation (21). Together, the resultsfrom these studies indicate that FKLF2 is able to activate transcriptionfrom many gene promoters via different sequenceelements.

Here we show that the coactivators CBP/p300 or PCAF stimulate transcriptional activation of the human $gamma$ globin promoter byFKLF2 in K562 cells. The acetyltransferase activity of PCAF butnot that of CBP/p300 is required for the stimulation of FKLF2activity, indicating that PCAF and CBP/p300 may play differentroles in coactivation with FKLF2. We further show that p300 andPCAF act cooperatively in stimulating FKLF2-mediated transcription.FKLF2 interacts with both CBP and PCAF through its zinc fingerdomain. FKLF2 interacts with specific regions of CBP and PCAF.Both CBP and PCAF acetylate FKLF2 in the zinc finger domain invitro. The binding of FKLF2 to the $gamma$ CACCC box was strongly stimulatedby CBP and PCAF. The histone acetyltransferase (HAT) activityof PCAF but not of CBP/p300 is required for stimulating FKLF2binding to the CACCC box of the $gamma$ promoter. Therefore, the functionalHAT domain of PCAF but not that of CBP/p300 is required both forstimulation of FKLF2 DNA binding and for coactivation of the $gamma$ promoter. Together with other studies, these results demonstratethat FKLF2 and other members of this family (such as EKLF) interactdifferentially with CBP/p300 or PCAF and that the activities ofthese family members are regulated by these coactivators throughdistinct mechanisms. The differential utilization of and regulationby CBP/p300 and PCAF may play important roles in the specificactivation of target genes by members of this highly conservedfamily of transcriptionfactors.

EXPERIMENTAL PROCEDURES

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Plasmids-- The plasmids pSG5DD and pSG5/FKLF2, which express the murine FKLF2, and the p $gamma$ luc and pHS₂ $beta$ luc reporter plasmids were as described(21). Expression plasmids for wild-type and HAT-defective PCAFwere provided by Y. Nakatani, T. Kouzarides, and I. Talianidis(20, 24, 25). Expression plasmids for wild-type p300 andHAT-defective p300 (D1485A/I1486L) were provided by A. Hecht (28).Expression plasmids for wild-type CBP and HAT-defective CBP (L1690K/C1691L)were provided by I. Talianidis (25). FKLF2-Myc plasmids thatexpress the full-length or a series of mutants of FKLF2 with aMyc tag at their C termini were constructed by inserting FKLF2or its mutants and a Myc tag into a mammalian expression vector.FLAG·CBP1 containing residues 451-662 and FLAG·CBP2 containingresidues 1680-1891 were constructed by inserting the correspondingPCR fragments and FLAG tag into a cytomegalovirus expression vector.GST·FKLF2 fusion proteins were constructed by inserting the correspondingPCR fragments into pGEX-4T-1 (Amersham Biosciences, Inc.). Forproduction of GST·CBP fusion proteins, DNA sequences correspondingto the indicated regions of CBP (CBP1, CBP2, and CBP3) were amplifiedby PCR, and the corresponding PCR fragments were inserted intopGEX-4T-1. GST fusion proteins containing wild-type or HAT-defectivePCAF were constructed by inserting their corresponding PCR fragments(amino acid residues 352-832) into pGEX-4T-1. GST fusion proteinscontaining the wild-type or mutant HAT domains of CBP (GST·CBP-HAT,residues 1196-1781) was constructed by inserting the correspondingfragments into pGEX-4T-1.

EMSA Assays-- EMSA assays were essentially as described (27) using purified GST fusion proteins and synthetic oligo probes containingthe distal CACCC box of the human $gamma$ globinpromoter.

Transfection and Luciferase Assays-- K562 cells cultured in 12-well plates were transfected using FuGENE 6 (Roche Molecular Biochemicals). Cells were harvestedat 36 h after transfection. Luciferase activity was measured usingthe Promega luciferase assaysystem.

Cell Extracts and Protein Purification-- Whole cell extracts from COS cells were prepared as described (27). GST fusion proteins were purified as described (27).The concentration and purity of the fusion proteins were determinedby SDS-PAGE and Coomassie Blue staining using bovine serum albuminasstandard.

In Vitro Protein Interaction Assays-- Whole cell extracts from COS cells expressing Myc-tagged FKLF2 were incubated with the GST·CBP or GST·PCAF fusion proteinsimmobilized on glutathione-agarose beads in a binding buffer containing20 mM Tris-HCl (pH 7.9), 10% glycerol, 100 mM KCl, 5 mM MgCl₂,0.5 mM EGTA, 0.5 mM EDTA, 2 mM dithiothreitol, and 0.2% IGEPAL-CA-630(Sigma) with protease inhibitors. The binding mixture was incubatedat 4 °C for 2 h. Beads were washed four times with 500 µl of bindingbuffer, resuspended in SDS sample buffer, and boiled for 5 min,and proteins were separated on 10% SDS-PAGE and transferred tonitrocellulose membrane. Myc·FKLF2 was detected using anti-Myc9E10 monoclonal antibody (Santa Cruz Biotechnology) and chemiluminescence(ECL, Amersham Biosciences, Inc.),respectively.

Coimmunoprecipitation Assays-- COS cells in 100-mm dishes were transfected with the FLAG·CBP, FLAG·CBP1, CBP2, or FLAG·PCAF expression vector together withthe Myc·FKLF2 expression plasmid as indicated using LipofectAMINE(Invitrogen). Coimmunoprecipitation assays were performed as described(30), except that the binding and washing buffers contained100 mM KCl. The presence of FKLF2 and the CBP or PCAF complexwas detected by immunoblotting using the anti-FLAG M2 monoclonalantibody (Sigma) or an anti-Myc 9E10 monoclonal antibody andchemiluminescence.

Protein Acetyltransferase Assays-- Protein acetyltransferase assays were carried out in reaction mixtures (30 µl) containing 50 mM HEPES (pH 8.0), 10% glycerol,50 mM KCl, 2 mM dithiothreitol, 10 mM sodium butyrate, 1 µl of[¹⁴C]acetyl-CoA, 1 µg of purified GST·FKLF2 fusion protein on beads,and 50 ng of purified GST·CBP-HAT containing the HAT domain ofCBP (residues 1196-1718), GST·PCA wild-type, or the GST·PCAF-HAT-defectivemutant. After incubating at 30 °C for 1 h with gentle mixing,the reaction mixtures were subjected to SDS-PAGE electrophoresisand analyzed using aphosphorimager.

RESULTS

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

CBP/p300 Function as Transcriptional Coactivators of FKLF2-- To understand the molecular mechanisms by which FKLF2 activates transcription, we determined whether CBP/p300 acts as an FKLF2coactivator and potentiates transcriptional activity in K562 cells.As expected from previous studies (21), FKLF2 activated the $gamma$ globin promoter. FKLF2 activity was further enhanced by CBP(Fig. 1). CBP by itself showed no effect on the $gamma$ globin promoter-drivenluciferase expression, indicating a functional interaction betweenCBP and FKLF2 at the $gamma$ globin promoter in vivo. These resultsdemonstrate that CBP functions as a coactivator for FKLF2 (Fig1).

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Fig. 1. CBP potentiates the transcriptional activity of FKLF2. K562 cells cultured in 12-well plates were transfected with 500 ng of the human $gamma$ globin promoter containing luciferase reporter p $gamma$ luc, 20 ng of empty vector (FKLF2) or FKLF2 expression vector (FKLF2⁺) and 200 ng of empty vector (CBP) or CBP expression vector (CBP⁺) as indicated. The results are presented as the mean ± S.D. (n = 3) of the relative light unit.

CBP and FKLF2 Interact in Vitro and in Vivo-- We next determined whether FKLF2 physically interacts with full-length CBP in vivo by a coimmunoprecipitation assay usingwhole cell extracts from COS cells expressing FLAG-tagged full-lengthCBP and Myc-tagged FKLF2. As shown in Fig. 2A, immunoprecipitationwith the anti-Myc antibody revealed the complex formation betweenCBP and FKLF2 in vivo. Reciprocal immunoprecipitation using anti-FLAGantibody also revealed the specific interaction between FKLF2and CBP (Fig. 2B). Fig. 2, C and D show that the FLAG-tagged CBPand Myc-tagged FKLF2 are expressed at similar levels. These datademonstrate that FKLF2 associates with full-length CBP in vivo(Fig. 2).

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Fig. 2. FKLF2 interacts with full-length CBP in vivo. Coimmunoprecipitation assays were performed using whole cell extracts from COS cells expressing FLAG-tagged full-length CBP (CBP-F) and Myc-tagged FKLF2 (FKLF2-M). A, immunoprecipitation with an anti-Myc antibody revealed the presence of CBP in the immunoprecipitate. B, reciprocal immunoprecipitation using anti-FLAG antibody also revealed that FKLF2 specifically interacts with CBP. C and D, FLAG-tagged CBP and Myc-tagged FKLF2 are expressed at similar levels. The asterisks indicate immunoglobin chains. IP, immunoprecipitation; IB, immunoblotting.

CBP contains distinct domains that interact with transcription factors. The CBP domains and some of their interacting proteinsare illustrated in Fig. 3A. GST fusion proteins containing differentregions of CBP were tested for their ability to interact withFKLF2. A GST pull-down assay was performed on GST·CBP fusion proteinsand whole cell extracts prepared from COS cells expressing Myc-taggedFKLF2. As shown in Fig. 3A, this assay revealed that FKLF2 interactsspecifically with CBP2, which is also essential for interactionswith factors including E1a, c-Fos, PCAF, MyoD, GATA-1, and TFIIB(17). The observed specific interaction of FKLF2 with CBP2 butnot CBP1, CBP3, and GST is not due to a difference in the amountof these fusion proteins used in the assay, because the same amountof each protein was included in the reaction as determined bySDS-PAGE and Coomassie Blue staining (data not shown). To determinethe in vivo association between FKLF2 and CBP2, coimmunoprecipitationassays were carried out using whole cell extracts from COS cellsexpressing FLAG-tagged CBP1 or CBP2 and Myc-tagged FKLF2. As shownin Fig. 3B, immunoprecipitation with the anti-Myc antibody revealedthe complex formation between CBP2 and FKLF2 in vivo. Consistentwith the results from the GST pull-down assay shown in (Fig. 3A),no in vivo association between CBP1 and FKLF2 was detected (Fig.3B). Reciprocal immunoprecipitation using the anti-FLAG antibodyalso revealed the specific interaction between FKLF2 and CBP2(Fig. 3B). The FLAG-tagged CBP1, CBP2, and Myc-tagged FKLF2 areexpressed at similar levels (Fig. 3B).

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Fig. 3. FKLF2 interacts with CBP in vitro and in vivo. A, FKLF2 interacts specifically with CBP2. The top panel shows the schematics of CBP, some of its interacting proteins, and its protein interaction domains used in this study. The bottom panel shows the GST pull-down results. GST pull-down assays were carried out by incubating 10 µl of whole cell extracts prepared from COS cells expressing the Myc-tagged FKLF2 protein with 2 µg of purified GST·CBP fusion proteins immobilized on glutathione-agarose beads as indicated. The presence of FKLF2 was detected by immunoblotting using the anti-Myc 9E10 monoclonal antibody and chemiluminescence. B, FKLF2 interacts with CBP2 in vivo. Coimmunoprecipitation assays were performed using whole cell extracts from COS cells expressing FLAG-tagged CBP1 (CBP1-F) or FLAG-tagged CBP2 (CBP2-F) and Myc-tagged FKLF2 (FKLF2-M). Top left, immunoprecipitation with an anti-Myc antibody revealed the presence of CBP2 but not CBP1 in the immunoprecipitates. Top right, reciprocal immunoprecipitation using an anti-FLAG antibody also revealed that FKLF2 specifically interacts with CBP2. Bottom left and right, FLAG-tagged CBP1, FLAG-tagged CBP2, and Myc-tagged FKLF2 are expressed at similar levels. The asterisks indicate immunoglobin chains. C, FKLF2 interacts with CBP through its zinc finger domain. a, a schematic presentation of the domain structure of FKLF2 and a series of Myc-tagged FKLF2 proteins used in this study. b, GST pull-down assays were performed using whole cell extracts from COS cells expressing Myc-tagged FKLF2 proteins as indicated and a purified GST·CBP2 fusion protein immobilized on glutathione-agarose beads. Bound proteins were identified by immunoblotting using an anti-Myc 9E10 monoclonal antibody and chemiluminescence. c, Myc-tagged FKLF2 proteins used in this assay are expressed at similar levels. d, a GST pull-down assay was carried out using whole cell extracts from COS cells expressing Myc-tagged FKLF2-(149-289) as shown in c and GST·CBP1 or GST·CBP2 as in b. This assay revealed the specific interaction of FKLF2 with CBP2 but not with CBP1.

Like other members of the Sp1/KLF family, FKLF2 contains distinct domains including a proline-rich potential transactivationdomain in the N-terminal portion and three highly conserved zincfingers (DNA-binding domain) in the C-terminal portion (Fig. 3C).To determine which region of FKLF2 interacts with CBP, GST pull-downassays were carried out by incubating whole cell extracts preparedfrom COS cells expressing Myc-tagged wild-type or deletion mutantsof FKLF2 proteins with a purified GST·CBP2 fusion protein immobilizedon glutathione-agarose beads. As shown in Fig. 3C, the GST pull-downassay demonstrates that CBP2 interacts specifically with the zincfinger region of FKLF2. The Myc-tagged FKLF2 and its mutants usedin this assay are expressed at similar levels (Fig. 3C). To furtherestablish the interaction of the FKLF2 zinc finger region withCBP2, GST pull-down assays were carried out using whole cell extractsfrom COS cells expressing Myc-tagged FKLF2-(149-289) and GST·CBP1or GST·CBP2. This assay revealed a specific interaction of FKLF2-(149-289)with CBP2 but not with CBP1 (Fig. 3C). By establishing the specificinteraction of the FKLF2 zinc finger region with CBP2 but notCBP1, this result rules out the possibility that the observedinteraction of FKLF2-(149-289) with CBP2 is due to a nonspecificinteraction of the cysteine rich zinc finger region (Fig. 3).

The Acetyltransferase Activity of CBP/p300 Is Dispensable for Its Function as Coactivator for FKLF2-- In addition to the ability to function as an intermediary molecule by direct interaction with both transcription activatorsand the general transcription machinery (14), CBP/p300 has intrinsicHAT activity (18, 19). Nucleosome acetylation has been associatedwith chromatin remodeling and gene regulation (31-35). The acetylationof transcription factors by CBP/p300 has also been shown to modulatethe activity of these proteins at multiple levels, including DNAbinding, protein-protein interactions, stability, and nucleocytoplasmicshuttling (24, 25, 36). The acetyltransferase function ofCBP/p300 is required for the superactivation of EKLF (36). However,several studies have shown that the HAT activity of p300 is notrequired for coactivation with a number of transcription factors,including E2F, MyoD, $beta$ -catenin, and the HIV Tat protein (24, 28,37, and 38). Therefore, the exact role of the acetylase activityof CBP/p300 in the coactivation of these two proteins with transcriptionactivators remains unknown. We examined whether the HAT activityof CBP/p300 is required for the potentiation of FKLF2 transcriptionalactivity using a HAT-defective p300 (p300 HAT), which contains a DI to AL exchange of p300 residues 1485 and1486 and abolishes its HAT activity (Refs. 28 and 39 and datanot shown). Transient assays were carried out by cotransfectionof a reporter containing the $gamma$ globin promoter and the FKLF2 expressionplasmid together with expression vectors for either wild-typep300 or p300 HAT in K562 cells. As shown in Fig. 4A, p300 and FKLF2 coactivatedthe $gamma$ globin promoter. P300 alone showed no effect on the $gamma$ globinpromoter activity, indicating that its recruitment to the $gamma$ globinpromoter is mediated through functional interaction with FKLF2.Both the wild-type and the HAT-defective p300 are capable of stimulatingFKLF2 transcriptional activation of the $gamma$ globin promoter. A higherdegree of stimulation of FKLF2 activity by the HAT-defective p300was also observed. To further establish the requirement of CBP/p300-HATactivity for the stimulation of FKLF2 transcriptional activity,the wild-type CBP and the mutant CBP (CBP-HAT, L1690K/C1691L), which lack HAT activity (25, 40 and our datanot shown), were also tested for the ability to stimulate FKLF2activation of the p $gamma$ luc reporter in K562 cells. These assays alsoshowed that the HAT activity of CBP is not required for its coactivationof FKLF2 transcriptional activation (data not shown). Proteinassays demonstrated that the wild-type and mutant p300 are expressedat similar levels (data not shown). These results demonstratethat CBP/p300 functions as a coactivator for FKLF2 in the transcriptionalactivation of the $gamma$ globin promoter and that the HAT activityof CBP/p300 is dispensable for its function as a coactivator forFKLF2.

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Fig. 4. The histone acetyltransferase activity of PCAF but not of p300 is required for its function as coactivator of FKLF2. A, the acetyltransferase activity of p300 is not required for its function as a coactivator of FKLF2. K562 cells cultured in 12-well plates were transfected with 500 ng of the human $gamma$ globin promoter containing reporter p $gamma$ luc, 20 ng of empty vector (FKLF2) or FKLF2 expression vector (FKLF2⁺), and 100 ng of empty vector (empty), wild-type p300 (p300wt), or HAT-defective mutant p300 (p300 HAT) as indicated. The results are presented as the mean ± S.D. (n = 3) of the relative light unit (RLU). B, the acetyltransferase activity of PCAF is required for its function as coactivator of FKLF2. Similar assays were carried out as described in A except that 0.05 µg, 0.1 µg, or 0.2 µg of expression plasmid for wild-type (PCAFwt) or HAT-defective mutant PCAF (PCAF-HAT) was used. The results are presented as the mean ± S.D. (n = 3) of the RLU.

The Acetyltransferase Activity of PCAF Is Required for Its Function as a Coactivator for FKLF2-- PCAF is another member of the transcription coactivators with acetylase activity (20). Both CBP/p300 and PCAF have beenshown to function as coactivators for a number of transcriptionfactors, including p53, E2F, and the estrogen receptor (24,41-43). In contrast, CBP/p300 but not PCAF is required for coactivationwith the erythroid-specific transcription factors GATA-1 and EKLF(8, 44, 45). The results from these studies suggest thattranscription activators may have a differential requirement forCBP/p300 or PCAF coactivators. We therefore determined whetherPCAF also functions as a coactivator for FKLF2 in transcriptionalactivation of the $gamma$ globin promoter in K562 cells. Fig. 4B demonstratesthat PCAF stimulated FKLF2 activity in a dose-dependent manner.PCAF by itself showed no effect on the luciferase expression.We next determined whether the HAT activity of PCAF is requiredfor the potentiation of FKLF2 transcriptional activation usingHAT-defective PCAF, which contains a deletion of amino acids 497-526(24). The HAT-defective PCAF failed to stimulate the transcriptionalactivation of the human $gamma$ globin promoter by FKLF2. Transcriptionalactivation of the $gamma$ globin promoter by FKLF2 was reduced by theHAT-defective PCAF, indicating an inhibitory effect on FKLF2 transcriptionalactivation by PCAF-HAT (Fig. 4B). The inability of HAT-defective PCAF to coactivateFKLF2 transcriptional activation is not due to the differencein expression levels, because Western blot analysis showed thatthese two are expressed at same level (data not shown). By demonstratingthat PCAF-HAT cannot coactivate with FKLF2 at different concentrations andhas inhibitory effects when expressed at a higher level, the quantitativeassays shown in Fig. 4B further rule out the possibility thatthis is due to the differences in the expression levels of thewild-type and mutant PCAF. These results demonstrate that PCAFfunctions as a coactivator of FKLF2 and that the HAT activityof PCAF is required for its synergistic activation of $gamma$ globinpromoter with FKLF2 (Fig. 4).

PCAF Interacts with FKLF2 through Its Zinc Finger Domain-- The above transient reporter assays showed a functional interaction between PCAF and FKLF2. We next determined whether FKLF2physically interacts with PCAF and which region of FKLF2 interactswith PCAF. A coimmunoprecipitation assay demonstrated that FKLF2associates with PCAF in vivo (Fig. 5A). GST pull-down assays asshown in the Fig. 3C legend were carried out by incubating wholecell extracts prepared from COS cells expressing Myc-tagged wild-typeor deletion mutant FKLF2 proteins (shown in Fig. 3C) with a purifiedGST·PCAF fusion protein. This assay demonstrated that PCAF interactswith the zinc finger domain of FKLF2 (Fig. 5B). GST·CBP2, whichhas been shown to interact with FKLF2 (Fig. 3C), was includedin parallel as a positive control. Although the data presentedhere are not quantitative, the strength of the signal generatedbetween FKLF2-(149-289) and GST·CBP2 is comparable with that generatedbetween FKLF2(149-289) and GST·PCAF under the conditions thatthe same amounts of FKLF2-(149-289) and GST·CBP2 or GST·PCAF wereused. These results demonstrated that FKLF2 physically contactsPCAF (Fig. 5).

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Fig. 5. FKLF2 interacts with PCAF in vivo and in vitro. A, FKLF2 interacts with PCAF in vivo. Coimmunoprecipitation assays were performed using whole cell extracts from COS cells expressing FLAG-tagged PCAF (PCAF-F) and Myc-tagged FKLF2 (FKLF2-M). Top left, immunoprecipitation with an anti-Myc antibody revealed the presence of PCAF in the immunoprecipitates. Top right, reciprocal immunoprecipitation using an anti-FLAG antibody also revealed that FKLF2 specifically interacts with PCAF. Bottom left and right, FLAG-tagged PCAF and Myc-tagged FKLF2 are expressed at similar levels. B, FKLF2 interacts with PCAF through its zinc finger domain. GST pull-down assays were performed as described in the Fig. 3C legend using whole cell extracts from COS cells expressing Myc-tagged FKLF2 proteins as indicated and a purified GST·PCAF fusion protein immobilized on glutathione-agarose beads. The interaction between CBP2 and FKLF2-(149-289) was included in the assay as positive control. The asterisk indicates nonspecific signals.

PCAF and p300 Act Synergistically in Stimulating FKLF2-driven Transcription-- Having established that both CBP/p300 and PCAF stimulated FKLF2 activity when individually co-expressed with FKLF2, we soughtto investigate whether PCAF and CBP/p300 act cooperatively instimulating FKLF2 transcription. Cotransfection experiments werecarried out in K562 cells using a $gamma$ globin promoter-driven luciferasereporter and the expression plasmids for FKLF2, PCAF, and p300or their respective empty vectors. This assay revealed that theinclusion of PCAF further stimulated transcription driven by FKLF2and p300 (Fig. 6). This cooperative activation also requires theacetylase activity of PCAF, because no stimulation was observedwhen the acetylase-defective PCAF was used (Fig. 6). Instead,a slight decrease in luciferase activity was found, indicatingan inhibitory effect on FKLF2 and p300 coactivation by an acetylase-defectivePCAF (Fig. 6).

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Fig. 6. The cooperative activation of the human $gamma$ globin promoter by FKLF2, PCAF, and p300. K562 cells cultured in 12-well plates were transfected with 500 ng of the human $gamma$ globin promoter containing reporter p $gamma$ luc, 20 ng of empty vector (FKLF2) or FKLF2 expression vector (FKLF2⁺), and 100 ng of empty vector, the expression vector for p300, PCAF, or HAT-defective mutant PCAF (PCAFHAT) as indicated. The results are presented as the mean ± S.D. (n = 3) of the relative light unit (RLU).

The Acetylation of FKLF2 by PCAF and CBP-- FKLF2 is an acetylated protein in vivo when expressed in COS cells (data not shown). To test whether PCAF and CBP acetylateFKLF2, acetylation assays were performed using purified GST fusionproteins of FKLF2, PCAF-HAT, and CBP-HAT. FKLF2 contains 13 lysineswith 11 of them located in the zinc finger DNA-binding domain.The N-terminal portion of FKLF2 (amino acids 1-160, containingtwo lysine residues) was not detectably acetylated by CBP andwas acetylated very weakly by PCAF (data not shown). To furtherdefine the sequences in the zinc fingers that are acetylated,we divided the zinc fingers of FKLF2 into two portions, and eachwas subjected to an acetylation assay. The N-terminal half fromamino acids 149 to 206 containing five lysine residues was acetylatedby CBP but not by PCAF. The C-terminal half from amino acids 200to 289 containing six lysines residues was acetylated by bothCBP and PCAF (Fig. 7). These results indicate that FKLF2 is apossible target of CBP/p300 and PCAF acetylation (Fig. 7).

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Fig. 7. FKLF2 was acetylated by both CBP and PCAF in vitro. An in vitro acetylation assay was carried out using purified GST fusion proteins of CBP-HAT-(1196-1718), PCAF-(352-832), and FKLF2-(149-289) containing the zinc finger domain of FKLF2, FKLF2-(149-206), and FKLF2 (200-289). The reaction mixtures were subjected to SDS-PAGE electrophoresis and autoradiography.

CBP/p300 and PCAF Stimulate FKLF2 Binding to the CACCC Box of the $gamma$ Promoter, and the Integrity of the HAT Domain of PCAF but Not That of CBP/p300 Is Required for the Stimulation of FKLF2 DNA Binding.-- To study the mechanisms by which the CBP/p300 and PCAF coactivators stimulate FKLF2 transcription activity, we first determinedwhether they increase the DNA binding activity of FKLF2 usingquantitative EMSA assays. As shown in Fig. 8A, the DNA bindingactivity of FKLF2 was strongly enhanced by both GST·CBP-HAT andGST·PCAF but not by GST alone. We next determined whether theHAT activity of CBP and PCAF is required for stimulating FKLF2binding to the $gamma$ CACCC box. As shown in Fig. 8B, GST·CBP-HAT stimulated FKLF2 DNA binding activity as well as the wild-typeCBP-HAT. In contrast, the HAT-defective mutant of PCAF stimulatedFKLF2 DNA binding very weakly (4-fold as comparing with the nearly20-30-fold stimulation by the wild-type PCAF, wild-type CBP, orCBP-HAT). The requirement of the integrity of the HAT domain of PCAFbut not that of CBP for stimulating FKLF2 DNA binding as shownby EMSA assays is consistent with the cotransfection assays, whichalso showed the requirement of the HAT activity of PCAF but notCBP/p300 for coactivation with FKLF2 (Fig. 4, A and B). GST·CBP-HAT,GST·CBP-HAT, GST·PCAF wild-type, or GST·PCAF-HAT alone showed no binding to the $gamma$ CACCC box-containing probe (datanot shown). In summary, these results demonstrate that the coactivatorsCBP/p300 and PCAF coactivate FKLF2 transcriptional activationof the $gamma$ promoter, at least in part by stimulating its bindingto the CACCC box of the $gamma$ promoter and that the integrity of theHAT domain of PCAF but not that of CBP/p300 is required for stimulatingFKLF2 DNA binding and transcriptional activity (Fig. 8).

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Fig. 8. CBP/p300 and PCAF stimulate FKLF2 DNA binding activity. A, a quantitative EMSA assay was carried out using purified CBP/p300 and PCAF stimulate FKLF2 DNA binding activity. A quantitative EMSA assay was carried out using purified GST·FKLF2-(149-289), GST, GST·CBP-HAT (residues 1196-1718), GST·PCAF (residues 352-832), and an oligonucleotide probe containing the distal CACCC box of the $gamma$ promoter. Lanes 2-4, 5-7, 8-10, and 11-13 received 1, 2, and 3 ng of GST·FKLF2-(149-289), respectively. Lanes 5-7, 8-10, and 11-13 also received 100 ng of GST, GST·CBP-HAT, and GST·PCAF, respectively. The concentration and purity of the GST fusion proteins were determined by SDS-PAGE and Coomassie Blue staining. The fusion proteins were purified to more than 95% purity (data not shown). B, the integrity of the HAT domain of PCAF but not of CBP is required for the stimulation of FKLF2 DNA binding activity. An EMSA assay was carried out using purified GST·FKLF2-(48-289) lacking the N-terminal 47 amino acid residues of FKLF2, GST·CBP-HAT (residues 1196-1718), GST·CBP-HAT (residues 1196-1718 containing L1690K/C1691L), wild-type GST·PCAF (residues 352-832), HAT-defective GST·PCAF-HAT (residues 352-832 containing Y616A/F617A), and an oligonucleotide probe containing the distal CACCC box of the $gamma$ promoter. Lanes 2-14 received 5 ng of GST·FKLF2-(48-289). Lanes 3-5, 6-8, 9-11, and 12-14 received 20 ng, 40 ng, and 80 ng of GST·CBP-HAT, GST·CBP-HAT, PCAF wild-type, and PCAF-HAT, respectively. The concentration and purity of the GST fusion proteins were determined by SDS-PAGE and Coomassie Blue staining. The fusion proteins were purified to more than 95% purity (data not shown). The asterisks indicate shifts that may be generated by truncated forms of GST·FKLF2. The filled arrow indicates the shift by the full-length GST·FKLF2(48-289), and the empty arrow indicates the free probe.

	DISCUSSION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

CBP/p300 functions as a coactivator for many transcription activators (15). CBP/p300 also has intrinsic acetyltransferaseactivities (18, 19). The acetylation of histone and transcriptionfactors by CBP/p300 has been implicated in the regulation of geneexpression (15, 31). At present, however, the exact role ofthe HAT activity of CBP/p300 in coactivation with transcriptionactivators remains to be established. For example, the HAT activityof p300 is not required for coactivation of the siamois promoterby p300 and $beta$ -catenin in 293 cells (28). The HAT activity ofp300 is also dispensable for its function as a coactivator forMyoD (38). Other studies have shown that the HAT activity ofp300 is not required for its function as a coactivator for HIVTat under integrated and nonintegrated conditions (37). Studieson the transcriptional activation by hepatocyte nuclear factor1 (HNF-1) showed that the HAT activity of PCAF but not that ofCBP/p300 is required for the stimulation of HNF-1 transcriptionunder a transient transfection assay. However, the HAT activitiesof both CBP/p300 and PCAF are important on a genome-integratedpromoter (25). Studies on KLF1/EKLF, the founding member ofthe family, demonstrated that the HAT activity of CBP/p300 isrequired for transcriptional superactivation with KLF/EKLF (36).We therefore tested whether the HAT activity of p300 is requiredfor its function as a coactivator for FKLF2 using a HAT-defectiveCBP/p300 (25, 28, 39). Our results showed that the HAT activityof CBP/p300 is not required for its coactivation of the human $gamma$ globin promoter with FKLF2. It was also noted that the HAT-defectivep300 showed a slightly higher stimulation of FKLF2 transcriptionactivity. Together, these studies indicate that different factorsmay have distinct requirements of the HAT activity of CBP/p300for their coactivation. The data presented here and in studiesby Zhang et al. (36) suggest that even members of the same familyof transcription factors have different requirements for the HATactivity of CBP/p300 and differential coactivation by CBP/p300and PCAF (see below). Further studies are needed to establishthe requirement for the HAT activity of CBP/p300 in the coactivationof the $gamma$ globin promoter with FKLF2 under chromosomalcontext.

PCAF is a member of a family of acetylases (48). PCAF exists in a complex of more than 20 polypeptides (49) and functionsas a coactivator for a number of transcription factors (15).Studies have shown that transcription factors may have selectivityin coactivation with coactivators. For example, CBP but not PCAFstimulates KLF1/EKLF transcriptional activity. We therefore determinedwhether PCAF functions as a FKLF2 coactivator. FKLF2 transcriptionalactivation of the $gamma$ globin promoter was further stimulated byco-expression of PCAF. By the use of PCAF harboring a deletionof residues 497-526 that abolishes its HAT activity (24), wedemonstrated that the HAT activity of PCAF is required for coactivationwith FKLF2. An inhibition of FKLF2 activation by HAT-defectivePCAF was observed at a higher expression level, indicating a possibledominant negative effect of the HAT-defective PCAF on FKLF2 transactivation.It has been shown that PCAF induces erythroid cell differentiation,and the expression of the $beta$ globin gene was stimulated by wild-typePCAF and inhibited by HAT-defective PCAF in erythroleukemia cells(50). The HAT activity of PCAF was also required for coactivationwith E2F, MyoD, and the Tat protein (18, 24, 38).

The results showing that both CBP/p300 and PCAF function as coactivators for FKLF2 whereas CBP but not PCAF functions as acoactivator for EKLF (8) suggest that there may be selectiveutilization of coactivators among different members of the Sp1/KLFfamily. To further establish whether CBP/p300 and PCAF selectivelystimulate FKLF2 transcriptional activation of the $gamma$ promoter,we also tested the ability of these coactivators to stimulateEKLF transcriptional activation of the $gamma$ promoter. In agreementwith our previous results (21), EKLF activated the $gamma$ promoteronly marginally (2-fold), whereas FKLF2 activated the same reporter100-fold in parallel transient transfection assays (Ref. 21and data not shown). This marginal activation of the $gamma$ promoterby EKLF is not significantly stimulated by p300 or PCAF (datanot shown). Consistent with previous studies, EKLF strongly activatedthe $beta$ promoter (8, 51), and this activation of the $beta$ promoterwas further stimulated by p300 (Ref. 8 and data not shown).The differential interaction with coactivators may be one of themechanisms by which members of the Sp1/KLF family of transcriptionfactors accomplish their specificity. Given the differences inpromoter and coactivator selectivity and in the mechanisms bywhich coactivators stimulate their transcriptional activity, FKLF2and EKLF transcription factors may provide an excellent modelfor studying how coactivators modulate the activity of transcriptionfactors of the same family. These studies may shed significantlight on our understanding of tissue and developmental stage-specificexpression of the globingenes.

Protein-protein interaction studies show that CBP and PCAF physically interact with FKLF2 through the zinc finger region.Functional studies suggest that that both CBP and PCAF act cooperativelyin the coactivation of FKLF2 transcription. EMSA assays demonstratethat both CBP/p300 and PCAF strongly stimulated the DNA bindingactivity of FKLF2. The integrity of the HAT function of PCAF butnot that of CBP/p300 is required for the stimulation of FKLF2DNA binding. Consistent with the cooperative coactivation of FKLF2transcription in transient assays (Fig. 6), our preliminary quantitativeEMSA assays also showed that CBP and PCAF act cooperatively instimulating FKLF2 binding to the CACCC box of the $gamma$ promoter,as demonstrated by the stronger stimulation of FKLF2 DNA bindingby inclusion of both CBP-HAT and PCAF wild-type than either coactivatoralone. The observed cooperative stimulation of FKLF2 DNA bindingalso requires the integrity of the HAT domain of PCAF, since itis not observed with PCAF-HAT (data not shown), the same as with the cooperative stimulationof FKLF2transcription.

An acetylation assay showed that CBP acetylates the zinc finger region of FKLF2. The acetylation of p53 by p300 has been reportedto stimulate its DNA binding activity (52). However, our resultsdemonstrate that the HAT activity of CBP is not required for stimulatingFKLF2 DNA binding activity. Studies on EKLF also demonstratedthat the acetylation of EKLF by CBP has no effect on its DNA binding(36). We therefore tested whether the HAT-defective CBP canstimulate p53 binding to its target site. Our results showed thatthe HAT-defective CBP stimulated p53 DNA binding as well as theHAT wild-type CBP, demonstrating that the HAT activity of CBPis not required for stimulating p53 DNA binding (data not shown).The study in this report and other studies (8, 52) demonstratethat FKLF2, p53, and EKLF are the targets of CBP acetylation.The acetylase activity of CBP is not required for stimulatingFKLF2 and p53 DNA binding. Therefore, the biological significanceof the acetylation of these factors by CBP remains to be determined.The acetylation of EKLF enhanced its interaction with the SWI/SNFcomplex rather than its DNA binding (36). Further studies willdetermine whether the acetylation of FKLF2 and p53 by CBP alsoregulates their interaction with other proteins. PCAF acetylatesFKLF2 weakly in comparison with CBP. Nevertheless, the integrityof the HAT activity of PCAF is required for stimulating FKLF2transcriptional and DNA binding activity. There are at least twopossible explanations for the observed requirement of PCAF-HAT.First, the HAT-defective mutant may be defective in its interactionwith FKLF2. Second, the weak acetylation is sufficient to stimulateFKLF2 DNA binding. Our protein-protein interaction studies usingthe wild-type and HAT-defective PCAF demonstrated that FKLF2 interactswith both the PCAF-(352-832) wild-type and the HAT-defective mutantequally well (data not shown). By ruling out the first possibility,our results suggest that the acetylation of FKLF2 by wild-typePCAF is necessary for stimulating its transcriptional and DNAbindingactivity.

ACKNOWLEDGEMENTS

We thank Drs. Y. Nakatani and T. Kouzarides, I. Talianidis, and A. Hecht forplasmids.

	FOOTNOTES

^* This work was supported by grants from the NIDDK and the NHLBI, National Institutes of Health.The costs of publication ofthis article were defrayed in part by the payment of page charges.The article must therefore be hereby marked "advertisement" inaccordance with 18 U.S.C. Section 1734 solely to indicate thisfact.

^¶ To whom correspondence should be addressed: University of Washington, Division of Medical Genetics, Box 357720, Seattle, WA98195-7720. Tel.: 206-543-3526; Fax: 206-543-3050; E-mail: gstam@u.washington.edu.

Published, JBC Papers in Press, December 17, 2001, DOI 10.1074/jbc.M108826200

ABBREVIATIONS

The abbreviations used are: EKLF, erythroid Krüppel-like factor; CREB, cAMP-response element-binding protein; CBP, CREB-binding protein; FKLF2, fetal Krüppel-like factor 2; PCAF, p300/CBP-associated factor; HAT, histone acetyltransferase; GST, glutathione S-transferase; EMSA, electrophoretic mobility shift assay.

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Functional Interaction between Coactivators CBP/p300, PCAF, and Transcription Factor FKLF2*

Functional Interaction between Coactivators CBP/p300, PCAF, and Transcription Factor FKLF2^*